The monotony of transferrin and esterase electrophoretic patterns in pirarucu, Arapaima gigas (Schinz, 1822) from Santa Cruz Lake, Tefé River, Amazonas, Brazil

Starch gel electrophoresis was used for examining the transferrin gene locus (Tf) and two esterase gene loci (Est-1 and Est-D1) of a pirarucu (Arapaima gigas) population sample collected from Santa Cruz Lake, Tefé River, Amazonas, Brazil. The Tf locus was tentatively classified as being polymorphic, showing two double-banded patterns (Tf 12 and Tf 22) of the three theoretically expected ones (Tf 11, Tf 12 and Tf 22), presumably controlled by two co-dominant alleles, Tf 1 and Tf 2. The monotony detected in pirarucu Tf locus genotypes showing a very high proportion of the double-banded heterozygote pattern Tf 12 (95% of the sampled individuals) may indicate the possibility of their having come from representatives of the same brood begotten by a pair of fish, where a single-banded Tf 11 homozygote pattern male would have crossed with a single-banded Tf 22 homozygote pattern female, or vice versa. One zone of electrophoretic activity was detected in esterase, presumably controlled by a monomorphic Est-1 locus with the fixed allele Est-11 where all individuals showed the single-banded Est-111 homozygote pattern. Esterase-D also displayed one zone of electrophoretic activity, presumably controlled by a monomorphic Est-D1 locus with a fixed allele Est-D11 where all individuals revealed the single-banded Est-D111 genotype pattern. The monotony comprised by single-banded genotype patterns in both esterase systems tested may also indicate the possibility of the individuals from the sample examined having come from representatives of the same brood begotten by a pair of fish with both the male and female having the same genotypes.

Variabilidade genética em algumas criações comerciais brasileiras de escargots (Helix aspersa, Müller, 1774) / Genetic variation at eight isoenzyme loci in subpopulations of the edible snail (Helix aspersa, Müller, 1774)

Descreveram-se os marcadores isoenzimáticos e estimou-se a variabilidade genética de 20 subpopulações brasileiras de escargots (Helix aspersa). O estudo dos oito locos foi feito por eletroforese em gel de amido, em amostras com 30 indivíduos cada, obtidas em criatórios dos estados de Santa Catarina, São Paulo e Rio de Janeiro (uma, duas e 17 amostras, respectivamente). Observou-se polimorfismo nos locos das enzimas LAP, 6-PGD, PEP 2, PEP 1 e MDH, com três alelos nos três primeiros locos e dois nos demais. Os locos da ME, da SOD e da PGI apresentaram-se monomórficos. As freqüências gênicas de sete amostras ajustaram-se ao modelo de Hardy-Weinberg (P<0,05), e as de outras seis amostras ajustaram-se ao modelo de Wright (P<0,05), indicando que elas estão submetidas a diferentes regimes reprodutivos. Os desvios da panmixia para toda a população (F IT ) e dentro das subpopulações (F IS) não foram significativos (P³0,05). O desvio entre as subpopulações (F ST=0,0485) foi significativo (P<0,05) e apontou pequena diferenciação entre elas. As estimativas de diversidade total (Ht), entre subpopulações (Dst) e dentro das subpopulações (Hs), indicaram que a diversidade genética é reduzida e sua maior parte encontra-se dentro das subpopulações, sugerindo uma base genética estreita para essa população. As distâncias genéticas também foram pequenas, não permitindo a construção de um dendrograma.

Determination of insecticide susceptibility in Culex quinquefasciatus Say adults by rapid enzyme microassays.

Rapid enzyme microassays for the detection of resistance due to organophosphate and carbamate in individual field-collected strains of Culex quinquefasciatus adults were conducted. These tests allowed accurate differentiation by eye, on the basis of color changes of susceptible and resistant individuals. Two separate tests were conducted for the biochemical assays. In the insensitive acetylcholinesterase (AChE) test, acetylthiocholine iodide (ACTH) and 5,5-dithiobis-(2-nitrobenzoic acid) (DTNB) were used as substrate and coupling agent respectively. The resulting yellow chromophore indicated AChE activity. Test results showed that the color intensity decreased as increasing concentrations of propoxur were added, thereby confirming the susceptibility of the enzyme to inhibitor. Assay of non-specific esterase however, indicated elevated levels which were correlated with degree of malathion resistance. Electrophoretic data revealed the presence of 2 esterase bands in all strains. It was concluded that such a pattern was not contributory to malathion resistance in adults.

Filarial enzymes by the horizontal starch-gel electrophoresis technique.

In preliminary studies, on adult filarial parasites, difference in the electrophoretic pattern of glucosephosphate isomerase (GPI) of B. malayi, B. pahangi and the rat filarial worm, B. booliati, was demonstrated. There also appears to be a difference in the GPI and lactate dehydrogenase isoenzyme patterns of B. malayi (subperiodic) from different animal hosts. These observations suggest that the zymogram technique may yet prove to be a sensitive taxonomic tool for use in the characterisation of filarial helminths. At present, the contention is that the subperiodic form of B. malayi exists as a zoonoses (possibly also with B. pahangi), which is drawn from findings backed by procedures that cannot easily differentiate between closely-related species and subspecies. Thus enzyme electrophoresis could complement the parasitological methods currently used, and contribute in enhancing the validity of this contention. More work, and on a larger scale to include the microfilariae and infective larvae, would be required.